CRISPR-Cas9-Mediated Precise Knock-In Edits in Zebrafish Hearts

清脆的 斑马鱼 基因组编辑 Cas9 生物 基因敲除 计算生物学 基因 遗传学 模式生物 正向遗传学 遗传筛选 表型
作者
Kyle E. Simpson,Shoaib Faizi,Ravichandra Venkateshappa,Mandy Yip,Raj Johal,Damon Poburko,Yen May Cheng,Diana Hunter,Eric Lin,Glen F. Tibbits,Tom W. Claydon
出处
期刊:Journal of Visualized Experiments [MyJOVE]
卷期号: (187) 被引量:1
标识
DOI:10.3791/64209
摘要

Clustered regularly interspaced short palindromic repeats (CRISPR) in animal models enable precise genetic manipulation for the study of physiological phenomena. Zebrafish have been used as an effective genetic model to study numerous questions related to heritable disease, development, and toxicology at the whole-organ and -organism level. Due to the well-annotated and mapped zebrafish genome, numerous tools for gene editing have been developed. However, the efficacy of generating and ease of detecting precise knock-in edits using CRISPR is a limiting factor. Described here is a CRISPR-Cas9-based knock-in approach with the simple detection of precise edits in a gene responsible for cardiac repolarization and associated with the electrical disorder, Long QT Syndrome (LQTS). This two-single-guide RNA (sgRNA) approach excises and replaces the target sequence and links a genetically encoded reporter gene. The utility of this approach is demonstrated by describing non-invasive phenotypic measurements of cardiac electrical function in wild-type and gene-edited zebrafish larvae. This approach enables the efficient study of disease-associated variants in a whole organism. Furthermore, this strategy offers possibilities for the insertion of exogenous sequences of choice, such as reporter genes, orthologs, or gene editors.

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